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首页> 外文期刊>Electrophoresis: The Official Journal of the International Electrophoresis Society >Poly(methyl methacrylate) microchip affinity capillary gel electrophoresis of aptamer-protein complexes for the analysis of thrombin in plasma.
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Poly(methyl methacrylate) microchip affinity capillary gel electrophoresis of aptamer-protein complexes for the analysis of thrombin in plasma.

机译:适体-蛋白质复合物的聚甲基丙烯酸甲酯微芯片亲和毛细管电泳,用于分析血浆中的凝血酶。

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Thrombin generation in blood serves as an important marker for various hemostasis-related diseases and conditions. Analytical techniques currently utilized for determining the thrombin potential of patients rely primarily on the enzymatic activity of thrombin. Microfluidic-based ACE using fluorescently labeled aptamers as affinity probes could provide a simple and efficient technique for the real-time analysis of thrombin levels in plasma. In this study, aptamers were used for the analysis of thrombin by affinity microchip CGE. The CGE used a poly(methyl methacrylate) (PMMA) microfluidic device for the sorting of the affinity complexes with a linear polyacrylamide (LPA) serving as the sieving matrix. Due to the fact that the assay was run under nonequilibrium electrophoresis conditions, the presence of the sieving gel was found to stabilize the affinity complex, providing improved electrophoretic performance compared to free-solution electrophoresis. Two fluorescently labeled aptamer affinity probes, HD1 and HD22, which bind to exosites I and II, respectively, of thrombin were investigated. With an electric field strength of 300 V/cm, two well-resolved peaks corresponding to free aptamer and the thrombin-aptamer complex were obtained in less than 1 min of separation time with a run-to-run and chip-to-chip reproducibility (RSD) of migration times <10% using both aptamers. HD22 affinity assays of thrombin produced baseline-resolved peaks with favorable efficiency due to its higher binding affinity, whereas HD1 assays showed poorer resolution of the free aptamer and complex peaks. HD22 was used in determining the level of thrombin in human plasma. Assays were performed directly on plasma that was diluted to 10% v/v. Thrombin was successfully analyzed by microchip CGE at a concentration level of 543.5 nM for the human plasma sample.
机译:血液中凝血酶的生成是各种与止血有关的疾病和状况的重要标志。当前用于确定患者的凝血酶潜力的分析技术主要依赖于凝血酶的酶活性。使用荧光标记的适体作为亲和探针的基于微流体的ACE可以为血浆中凝血酶水平的实时分析提供一种简单有效的技术。在这项研究中,适体用于亲和微芯片CGE对凝血酶的分析。 CGE使用聚甲基丙烯酸甲酯(PMMA)微流控设备对亲和配合物进行分选,其中线性聚丙烯酰胺(LPA)用作筛分基质。由于该测定是在非平衡电泳条件下进行的,因此发现存在筛分凝胶可以稳定亲和复合物,与自由溶液电泳相比,电泳性能得到改善。研究了两种荧光标记的适体亲和力探针HD1和HD22,它们分别与凝血酶的I和II外突结合。在300 V / cm的电场强度下,在不到1分钟的分离时间内即可获得两个游离离子适体和凝血酶-适体复合物的良好分离峰,并具有连续运行和芯片间重复性的特点两种适体的迁移时间(RSD)<10%。凝血酶的HD22亲和力测定法具有较高的结合亲和力,可产生基线分离的峰,且效率较高,而HD1测定法显示的游离适体和复杂峰的分离度较差。 HD22用于测定人血浆中的凝血酶水平。直接在稀释至10%v / v的血浆上进行测定。通过微芯片CGE成功地分析了人血浆样品中的凝血酶浓度为543.5 nM。

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